key: cord-0819905-nacemmcb authors: Villegas-Gómez, Isaac; Silva-Olivares, Angélica; Robles-Zepeda, Ramón Enrique; Gálvez-Ruiz, Juan-Carlos; Shibayama, Mineko; Valenzuela, Olivia title: The Dichloromethane Fraction of Croton sonorae, A Plant Used in Sonoran Traditional Medicine, Affect Entamoeba histolytica Erythrophagocytosis and Gene Expression date: 2021-07-23 journal: Front Cell Infect Microbiol DOI: 10.3389/fcimb.2021.693449 sha: 69bb5a66213ecf3c239e32b95d84eef65899b456 doc_id: 819905 cord_uid: nacemmcb Intestinal parasites are a global problem, mainly in developing countries. Obtaining information about plants and compounds that can combat gastrointestinal disorders and gastrointestinal symptoms is a fundamental first step in designing new treatment strategies. In this study, we analyzed the antiamoebic activity of the aerial part of Croton sonorae. The dichloromethane fraction of C. sonorae (CsDCMfx) contained flavonoids, terpenes, alkaloids, and glycosides. The ultrastructural morphology of the amoebae treated for 72 h with CsDCMfx was completely abnormal. CsDCMfx reduced erythrophagocytosis of trophozoites and the expression of genes involved in erythrocyte adhesion (gal/galnac lectin) and actin cytoskeleton rearrangement in the phagocytosis pathway (rho1 gtpase and formin1). Interestingly, CsDCMfx decreased the expression of genes involved in Entamoeba histolytica trophozoite pathogenesis, such as cysteine proteases (cp1, cp4, and cp5), sod, pfor, and enolase. These results showed that C. sonorae is a potential source of antiamoebic compounds. Parasitic intestinal infections have medical and economic impacts worldwide, and it is estimated that three billion people are affected annually. Entamoeba histolytica is one of the most prevalent intestinal protozoa in the human gut and is the etiologic cause of amoebiasis and amoebic liver abscess (ALA), affecting approximately 50 million people and approximately 100,000 deaths annually (Stanley, 2003) . Amoebiasis is endemic in Mexico, and 187,785 cases were registered in 2019 (Secretarıá De Salud, 2019) . E. histolytica infection is established by parasite adherence to the colonic mucin layer and is capable of invasion of the large intestine, causing extensive tissue destruction and an important inflammatory reaction (Marie and Petri, 2014) . Without treatment, it can result in amoebic dysentery and ALA (Cornick et al., 2017) . Metronidazole (MTZ) is the most commonly used drug for E. histolytica intestinal infection and liver necrosis. In addition, strains resistant to MTZ have been reported, and MTZ can cause different secondary effects, such as diarrhea, nausea, headache, and teratogenic effects (Penuliar et al., 2015) . Through many generations, plants have been used to treat different diseases and their symptoms, including gastrointestinal disorders such as diarrhea, nausea, stomachache, colitis, and vomiting, which can be caused by parasites such as E. histolytica (Mi-Ichi et al., 2016) . In Sonoran traditional medicine, some ethnic groups, such as Mayos, Yaquis, Seris, Pimas, and Guarijios, have used certain plants to treat gastrointestinal disorders and gastrointestinal symptoms (Moreno-Salazar et al., 2008) . Some compounds isolated from the Croton species, mostly terpenoids, glycosides, alkaloids, a few flavonoids and others (dos Santos et al., 2015; Xu et al., 2018) , have antiproliferative, antifungal, antibacterial and antiparasitic activities (Noor Rain et al., 2007; Adelekan et al., 2008; Guimarães et al., 2010; Obey et al., 2018) . In the Croton genus, more than 300 terpenoids have been identified and characterized (Xu et al., 2018) . Velaźquez-Domıńguez et al. (2013) reported a sesquiterpene lactone incomptine A, with an amoebicidal effect on E. histolytica. Other reports have demonstrated in vitro amoebicidal properties of essential oils of the aerial parts of some Croton species (rich on sesquiterpenes) against trophozoites of Acanthamoeba polyphaga (Vunda et al., 2012) . Flavonoids (Resveratrol) can induce oxidative stress, dysregulation of glycolytic enzymes, and apoptosis-like death in E. histolytica trophozoites (Pais-Morales et al., 2016) . Additionally, some studies have shown that the main molecular targets correspond to cytoskeleton-related proteins such as myosin II, actin and a-actin, modifying pathogenic mechanisms such as adhesion, cytolysis, phagocytosis and migration (Bolaños et al., 2014; Bolaños et al., 2015; Pais-Morales et al., 2016) . The actin cytoskeleton is an important virulence factor in E. histolytica that is involved in phagocytosis for nutrient intake and invasion (Aslam et al., 2012) . Rho GTPases and their downstream effectors, such as formin, regulate cytoskeletal reorganization in various cellular processes, such as cytokinesis, motility, and apoptosis (Hall, 1998) . E. histolytica expresses a family of eight formins; Ehformin 1 and 2 have been shown to interact with microtubule assembly in the nucleus and regulate mitosis and cytokinesis in E. histolytica (Majumder and Lohia, 2008) . Approximately 50 cysteine proteases (cps) genes present in the E. histolytica genome (Irmer et al., 2009) , and the expression is different when the trophozoites analyzed were obtained from in vitro culture versus in vivo infection (He et al., 2010) and are essential for mucus degradation and for the degradation of phagocytosed cells or debris (Nakada-Tsukui et al., 2012) . The E. histolytica death process is not well understood, and this organism has noncanonical caspases (Pais-Morales et al., 2016) , but calpain-like protein activity increases when programmed cell death (PCD) is induced by nitric oxide species (NOS) (Ramos et al., 2007; Villalba et al., 2007; Nandi et al., 2010; Domıńguez-Fernańdez et al., 2018) . In this study, we analyzed the antiamoebic activity of the aerial part of Croton sonorae. The dichloromethane fraction of C. sonorae contained the most effective compounds against E. histolytica trophozoites, demonstrating an effect on erythrophagocytosis and affecting the gene expression of some proteins involved in the pathogenesis of this amoebae. Croton sonorae was collected at the location 29°09'03.00" N, 110°5 6'59.51" W, with classification number 21,420. This plant was authenticated by Professor JoséJesuś Sańchez Escalante, and a voucher specimen number was later deposited in the Herbarium of the University of Sonora. The aerial part of C. sonorae was dried at room temperature for at least 2 weeks. The dried plant material was powdered and mixed with methanol (1:10 w/v) for 10 days, and the resulting extract was evaporated under reduced pressure (Jimeńez-Estrada et al., 2013) . The C. sonorae extract was fractionated using methanol, hexane, ethyl acetate and dichloromethane (DCM). Amoebic Culture E. histolytica HM1:IMSS, kindly donated by Dr. Mineko Shibayama, was cultured axenically at 37°C in TYI-S-33 medium supplemented with 20% (v/v) heat-inactivated bovine serum and 10% (v/v) diamond vitamin-Tween 80 solution (Diamond et al., 1978) . Trophozoites in the log phase of growth were placed on 24-well plates with different initial inoculum, 4 × 10 4 , 6 × 10 4 , 8 × 10 4 and 1 × 10 5 trophozoites/well in triplicate (were kept in BD GasPack jars), and counted in a hemocytometer every 24 until 96 h. Viability was measured with trypan blue exclusion dye (Penuliar et al., 2015) . For all assays, harvested E. histolytica trophozoites in log phase were placed on 24-well plates (6 × 10 4 trophozoites/well) in the presence of different concentrations of crude extracts (200 and 500 mg/ml) or fractions (18.75-300 mg/ml) and incubated at 37°C for 24, 48 and 72 h. Dimethyl sulfoxide (DMSO) was used as the solvent control, MTZ at 0.25 mg/ml was used as the amoebicidal drug control, and trophozoites with complete medium were used as the growth control. All wells had a final volume of 2.3 ml with complete medium. After incubation, trophozoites were detached by chilling in ice water for 30 min and counted on a hemocytometer. The viability was measured with trypan blue exclusion dye. The IC 50 was calculated by probit analysis in IBM ® SPSS ® Statistics v. 25. E. histolytica trophozoites in the log phase of growth were harvested and incubated in 24-well plates (6 × 10 4 trophozoites/well) with DMSO (0.1%), MTZ (0.25 mg/ml) or C. sonorae DMC fraction (118 mg/ml) every 24, 48 and 72 h. Trophozoites were washed twice with TYI-S-33 medium without supplementation and coincubated with human erythrocytes (1:100) every 30 min. Erythrophagocytosis was stopped with 4% paraformaldehyde to fix trophozoites. Phagocytized erythrocytes were counted in at least 80 amoebae per well. Trophozoites grown in complete medium were set as 100% erythrophagocytosis (Mora-Galindo et al., 2004) . To analyze ultrastructural changes, trophozoites treated with the C. sonorae fraction at 118 mg/ml (CsDCMfx) were harvested after 24, 48 and 72 h, washed twice with PBS (pH 7.2) and fixed with 2.5% glutaraldehyde in 0.1 M. Postfixation was performed with 2% osmium tetroxide. The samples were dehydrated with increasing concentrations of ethanol (70, 80, 90, 100%) and finally with propylene oxide. Subsequently, the amoebae were embedded in epoxy resin. Semithin sections (0.5 µm) were stained with toluidine blue and observed under a light microscope (Eclipse 80i microscope, Nikon, Japan). Fine sections (80 nm thick) were contrasted with uranyl acetate and lead nitrate and observed with a JEOL-JEM 1400 TEM (Pais-Morales et al., 2016). Total RNA was extracted from E. histolytica trophozoites after 24, 48 or 72 h of incubation with DMSO (0.1%), MTZ (0.25 mg/ ml), CsDCMfx (118 mg/ml) or only complete medium (control) using an Arcturus PicoPure RNA Isolation Kit (Thermo Fisher Scientific, Lithuania) following the manufacturer´s instructions. After RNA quantification with a NanoDrop spectrophotometer, amplification of mRNA transcripts was performed using 100 ng of total RNA for the calpain gene and 0.1 ng for actin, formin1, gal/galnac lectin, rho1, atg8, sod, enolase, pfor, cp1, cp2, cp4, and cp5. qPCR with a SYBR Green RT-PCR one-step kit (Agilent, USA) was used. The primers used for amplification are shown in Supplementary Figure 1 with actin as the reference gene. The PCR cycling conditions consisted of an initial step of 10 min at 50°C and 3 min at 95°C for all genes followed by 40 cycles of denaturalization at 95°C for 10 s and annealing at 60°C for 5 s for the actin (Majumder and Lohia, 2008) , formin1 (Majumder and Lohia, 2008) , gal/galnac lectin (Ximeńez et al., 2017) , rho1 (Bosch et al., 2011 ), calpain (Domıńguez-Fernańdez et al., 2018 , sod (Ximeńez et al., 2017) , enolase (Segovia-Gamboa et al., 2011) and pfor (Tazreiter et al., 2008) genes; 40 cycles of denaturalization at 95°C for 10 s, annealing at 52°C for 30 s and extension at 72°C for 30 s for atg8 (Picazarri et al., 2015) . The Ct values and the 2 −DCt formula were used for quantification (Livak and Schmittgen, 2001) . It has been observed that pathogenic strains of E. histolytica trophozoites incur a fitness cost reflected in the doubling time in vitro (Calzada et al., 1998; Penuliar et al., 2015) , which is longer than that of nonpathogenic strains and can be different between pathogenic strains. Due to these differences, it was necessary to construct a proliferation curve with different initial inocula (4, 6, 8 and 10 × 10 4 trophozoites/well) counted every 24 until 96 h. The growth curve of E. histolytica showed that at 72 h, a maximum peak of growth was observed at 6, 8 and 10 × 10 4 trophozoites/well, and the viability in all assays was greater than 95%, diminishing to almost half of the number of trophozoites at 96 h with viability under 90% (Supplementary Figure 1) . The initial inoculum of 4 × 10 4 trophozoites/well was discarded as an option to perform our experiments because it had a peak number of trophozoites at 96 h with viability under 90% (Supplementary Figure 1) . Using the formula for doubling time in E. histolytica HM1:IMSS in this study, we obtained 26.05 ± 0.82 h until log phase (72 h) with 6 × 10 4 trophozoites/well as the initial inoculum, and it was less variable between times for each initial inoculum, according to the growth curve (Supplementary Figure 1) . Similar results were observed by Penuliar et al. (2015) using the same pathogenic strain (Penuliar et al., 2015) . With these results, we selected 6 × 10 4 trophozoites/well for all experimental procedures. Antiparasitic Activity of C. sonorae Extract To investigate the amoebicidal activity, we first evaluated the mortality percentage at 200 mg/ml and 72 h for crude plant extract, and the mortality was less than 5% for the extract evaluated in comparison with the control; the diluent control (DMSO) produced only 2.85% death, and MTZ at 0.25 mg/ml was ≥95% (Supplementary Figure 2A ). Next, we tested 500 mg/ ml plant extract, and C. sonorae extract produced mortality greater than 95% (Supplementary Figure 2A) . To calculate the IC 50 by probit analysis, we tested the C. sonorae extract at 200, 350 and 500 mg/ml, resulting in an IC 50 = 306.23 mg/ml at 72 h. At 24 h with the C. sonorae extract (200 mg/ml), the trophozoites were agglutinated (Supplementary Figure 2B) , but at higher concentrations (350 and 500 mg/ml), we observed increased mortality (Supplementary Figure 2A) ; at 72 h with the C. sonorae extract (200 mg/ml), trophozoites were smaller and rounded compared with control amoebae (Supplementary Figure 2B) . We fractionated the C. sonorae extract with four different solvents: hexane, methanol, ethyl acetate and DCM. We tested them initially at 306 mg/ml, and only the hexane and DCM fractions produced mortality rates greater than 80% at 72 h (86.2 and 97.6%, respectively). To obtain the IC 50 values for the hexane and DCM fractions, we tested 300, 150, 75, 37.5 and 18.75 mg/ml ( Figure 1A) . The calculated IC 50 values were 118.7 and 122.1 mg/ml for the DCM and hexane fractions, respectively. The agglutination effect of the extract was lost in the hexane and DCM fractions at each time point and at all tested concentrations, but the trophozoites treated with CsDCMfx were affected in terms of shape and size similar to the extract ( Figure 1B ). The ultrastructure of the amoebae was analyzed by TEM. We found abundant glycogen deposits following treatment for 24 and 48 h with CsDCMfx ( Figures 2C, D) , and morphologically the cells appeared rounded and smaller than the control (axenic amoebae) and DMSO-treated cells (Figures 2A, B, respectively) . The ultrastructural morphology of the amoebae treated for 72 h with CsDCMfx was completely abnormal, and lysis of the amoebae was evident ( Figure 2E The actin cytoskeleton provides shape and motility in E. histolytica trophozoites; actin is recruited in the zone of contact with other cells to form the phagocytic cup and phagocyte (Majumder and Lohia, 2008; Herrera-Martıńez et al., 2016) . Because the C. sonorae DCM fraction (CsDCMfx) affects the amoeba shape, we evaluated the phagocytic capability of trophozoites treated with CsDCMfx at 118 mg/ml for 24, 48 and 72 h. The phagocytic activity diminished significantly compared with control amoebae to 63.75% (SD ± 4.55%) at 24 h of treatment, then to 58.9% (SD ± 3.9%) and 35.73% (SD ± 2.26%) (48 and 72 h, respectively) ( Figure 3A ). The amoebae treated with CsDCMfx for 48 h exhibited reduced mRNA expression of formin1, gal/galnac lectin, A B FIGURE 1 | (A) Viability percentage of E histolytica trophozoites treated for 24, 48 and 72 h and cultivated with complete medium (control); MTZ was used as the drug control (0.25 mg/ml), DMSO as the diluent control (1%) and C. sonorae extract at different concentrations. (B) All samples were stained with trypan blue dye exclusion. 400×. Error bars represent SD. * means p <0.05 when compared with control. The blue bars represent control; orange bars represent DMSO; gray bars represent MTZ; yellow represent C. sonorae extract at 300 mg/ml; light blue represent C. sonorae extract at 150 mg/ml; green represent C. sonorae extract at 75 mg/ml; dark blue represent C. sonorae extract at 37.5 mg/ml; brown represent C. sonorae extract at 18.75 mg/ml. Croton Frontiers in Cellular and Infection Microbiology | www.frontiersin.org July 2021 | Volume 11 | Article 693449 superoxide dismutase (SOD), enolase, and pyruvate-ferredoxin oxidoreductase (pfor) and increased expression of Rho1, calpain and atg8 compared with control amoebae (Figure 4) . The amoebae treated with CsDCMfx for 72 h exhibited increased expression of calpain in comparison with the other genes ( Figure 4) . We observed a decrease in cps mRNA in trophozoites treated with CsDCMfx. To date, there has been no consensus regarding the cutoff point at which the concentration of an extract is considered to demonstrate good antiparasitic activity, as in the case of the antitumoral activity of extracts (<30 mg/ml) provided by the National Cancer Institute [33] . Here, we found that CsDCMfx is cytotoxic to E. histolytica trophozoites (IC 50 = 118.7 mg/ml). This effect is considered "moderate" according to antiamoebic extract classification (Calzada et al., 2006) ; however, this particular classification (IC 50 less than 20 µg/ml, the antiprotozoal activity was considered good, and from 20 to 150 µg/ml, the antiprotozoal activity was considered moderate) was defined by using a lower initial number of amoebae (6 × 10 3 ) in comparison with the numbers used in this study (6 × 10 4 ), which would underestimate the antiamoebic activity. We found the presence of some main secondary metabolite groups in the C. sonorae extract and CsDCMfx (Xu et al., 2018) . Both the extract and CsDCMfx contain flavonoids previously identified and characterized in the genus Croton (Xu et al., 2018) . It is known that some flavonoids can alter cytoskeletal functions in E. histolytica trophozoites and considerably diminish erythrophagocytosis activity (Bolaños et al., 2014; Bolaños et al., 2015) . We observed in our results that erythrophagocytosis in amoebas treated with CsDCMfx diminished (Figures 3A, B) . The proposed model for the role of Rho1 during phagocytosis in E. histolytica is that it recruits Formin1 by releasing it from an intramolecular inhibitory state. Formin1 dimerizes and forms F-actin filaments beneath the membrane to generate a phagocytic c u p ( M a j u m d e r a n d L o h i a , 2 0 0 8 ) . A c c o r d i n g t o erythrophagocytosis assay and expression of rho1 and formin1, the low expression of formin1 (−1.73-and −2.30-fold change) can be a factor involved in the lack of phagocytosis in treated amoebae at 48 and 72 h (58.9 and 35.73%, respectively). The gal/galnac lectin was downregulated −105.1-fold at 48 h in amoebae treated with CsDCMfx, and this lectin is one of the principal adherence proteins facilitating the phagocytosis of red blood cells in phagocytic assays, supporting the lack of erythrophagocytosis. At 72 h, trophozoites treated with CsDCMfx and gal/galnac lectin expressed a −38.7-fold change, the rho1 gene expressed a −175.6-fold change and formin1 expressed a −2.30fold change, explaining the lack of phagocytosis. It was demonstrated that in E. histolytica, upregulation of calpain-like genes occurs during programmed cell death (Domıńguez-Fernańdez et al., 2018) . In this study, calpain was overexpressed 1.33-and 27.97-fold in amoebae treated with CsDCMfx at 48 and 72 h, respectively, suggesting an induction of programmed cell death, but according to the changes observed by TEM at 72 h, the amoebae died by lysis ( Figure 2E ). Autophagy is an intracellular degradation system that delivers cytoplasmic materials to the lysosome/ vacuole (Nishimura and Tooze, 2020) ; Entamoeba histolytica, possesses a restricted set of autophagy-related (Atg) proteins compared with other eukaryotes; Atg8 is considered to be the central and authentic marker of autophagosomes (Picazarri et al., 2015) . The Atg8 gene was overexpressed in trophozoites treated with CsDCMfx at 48 h by 9.01-fold change, and it was downregulated by −6.44-fold change at 72 h. In the Croton genus, more than 300 terpenoids have been identified and characterized (Xu et al., 2018) . Velaźquez-Domıńguez et al. (2013) reported a sesquiterpene lactone, incomptine A, with an amoebicidal effect on E. histolytica and in energy metabolism, downregulating the protein expression of enolase and PFOR enzymes. We found that pfor and enolase mRNA was downregulated in the amoebae treated with CsDCMfx for 48 and 72 h. SOD is the first line of defense against reactive oxygen species (ROS). SOD enzymes are a family of metalloenzymes responsible for quenching the potentially deleterious effects of superoxide radicals (Akbar et al., 2004) . Elevated levels of superoxide radicals result in higher expression on iron-containing sod (Akbar et al., 2004) . Our data showed downregulation of enolase and sod gene expression in amoebas treated with CsDCMfx at 48 h (−3.33-and −3.21-fold change, respectively). However, it is necessary to evaluate the presence of reactive oxygen species to confirm this evidence. Cysteine proteases (CPs) play a key role in cleavage and penetration into the intestinal lumen. The genes of these proteins are overexpressed in E. histolytica but absent or nonexpressed in E. dispar (Ximeńez et al., 2017) . Through these proteins, CP1, CP2 and CP5 are responsible for 90% of the cysteine protease activity in E. histolytica (Siqueira-Neto et al., 2018) . CP1 can digest collagen and adhere to enterocyte laminin, and it is located on the trophozoite surface and inside vacuoles (Nakada-Tsukui et al., 2012) . CP2 is located beneath the internal membrane, and on the amoeba surface, it is capable of degrading collagen and cartilage. CP2 has been observed to be overexpressed in vivo using a hamster model for ALA development. The important implication of CP5 in virulence has been demonstrated: it is able to degrade mucin on colonic explants and is unable to invade the intestinal epithelium when cp5 is silenced (Marie and Petri, 2014) . CPs are necessary for the degradation of phagocytosed material, and we observed downregulation of cps in trophozoites treated with CsDCMfx ( Figure 4) due to the lack of erythrophagocytosis. Further experiment will evaluate the proteinase activity to confirm the activity of CPs. We also performed a transmission electron microscopy analysis to assess ultrastructural changes in E. histolytica induced by CsDCMfx (118 µg/ml) at different times. For control amoebae, without treatment, the amoebae presented their typical morphology, and a normal nucleus, pseudopods and vacuoles were observed (Figure 2A ). E. histolytica trophozoites treated with 0.5% DMSO displayed normal morphology with several vacuoles and a nucleus containing peripheral chromatin ( Figure 2B ). After 24 and 48 h of treatment of E. histolytica with CsDCMfx, we observed several vacuoles of different morphologies and sizes, as well as increased glycogen stores. The continuity of the cytoplasmic membrane was preserved at these times ( Figures 2C, D) . After 72 h of treatment, disruption of the plasma membrane was evident, and glycogen and several vesicles were also observed ( Figure 2E ). Based on our transmission electron microscopy study, we believe that the mechanism of action of CsDCMfx against E. histolytica mainly affects the cytoplasmic membrane, causing lysis in the amoeba. We consider it important to continue with the search and isolation of bioactive compounds of CsDCMfx that allow the generation of new pharmaceutical alternatives to treat amoebiasis. In conclusion, the plant C. sonorae is a potential source of antiamoebic compounds. CsDCMfx was able to prevent erythrophagocytosis by downregulating gal/galnac lectin, which is necessary for adhesion to erythrocytes, and actin rearrangement via the Rho1 GTPase and Formin1 pathways. The original contributions presented in the study are included in the article/Supplementary Material. Further inquiries can be directed to the corresponding author. 4 | qRT-PCR of rho1, formin1, gal/galnac lectin, cp1, cp2, cp4, cp5, calpain, atg8, enolase, sod, and pfor. A 2 −DCT data analysis, taking C T values for actin expression as the reference gene. DCM means amoebae treated with CsDCMfx at 118 mg/ml. Error bars represent SD. * means p < 0.05 when compared with control. The authors wish to dedicate this manuscript to the memory of our friend and colleague Mineko Shibayama, whose life has been sadly claimed by the currently ongoing COVID-19 pandemic. The Bioactive Diterpenes and Other Constituents of Croton Steenkampianus Entamoeba histolytica The Calmodulin-like Calcium Binding Protein EhCaBP3 of Entamoeba histolytica Regulates Phagocytosis and Is Involved in Actin Dynamics Kaempferol Inhibits Entamoeba histolytica Growth by Altering Cytoskeletal Functions The Flavonoid (-)-Epicatechin Affects Cytoskeleton Proteins and Functions in Entamoeba histolytica Unique Structural and Nucleotide Exchange Features of the Rho1 Gtpase of Entamoeba histolytica Screening of Mexican Medicinal Plants for Antiprotozoal Activity In vitro Susceptibility of Entamoeba histolytica and Giardia lamblia to Plants Used in Mexican Traditional Medicine for the Treatment of Gastrointestinal Disorders Induced Mucin Exocytosis Is Mediated by VAMP8 and Is Critical in Mucosal Innate Host Defense A Calpain-Like Protein Is Involved in the Execution Phase of Programmed Cell Death of Entamoeba Histolytica Antiproliferative Activity of Flavonoids From Croton Sphaerogynus Baill. (Euphorbiaceae) Activity of the Julocrotine, a Glutarimide Alkaloid From Croton Pullei Var Rho GTPases and the Actin Cytoskeleton A Novel Entamoeba histolytica Cysteine Proteinase, EhCP4, Is Key for Invasive Amebiasis and a Therapeutic Target Strother and Its Effect on the Actin Cytoskeleton of Entamoeba histolytica Major Cysteine Peptidases of Entamoeba histolytica Are Required for Aggregation and Digestion of Erythrocytes But Are Dispensable for Phagocytosis and Cytopathogenicity In vitro Antioxidant and Antiproliferative Activities of Plants of the Ethnopharmacopeia From Northwest of Mexico Analysis of Relative Gene Expression Data Using Real-Time Quantitative PCR and the 2(-Delta Delta C(T)) Method Entamoeba histolytica Encodes Unique Formins, a Subset of Which Regulates DNA Content and Cell Division Regulation of Virulence of Entamoeba histolytica Entamoeba Encystation: New Targets to Prevent the Transmission of Amebiasis Entamoeba histolytica: Correlation of Assessment Methods to Measure Erythrocyte Digestion, and Effect of Cysteine Proteinases Inhibitors in HM-1:IMSS and HK-9:NIH Strains Plant Folk Medicines for Gastrointestinal Disorders Among the Main Tribes of A Novel Class of Cysteine Protease Receptors That Mediate Lysosomal Transport Hydrogen Peroxide Induces Apoptosis-Like Death in Entamoeba histolytica Emerging Roles of ATG Proteins and Membrane Lipids in Autophagosome Formation Antiplasmodial Properties of Some Malaysian Medicinal Plants Antimalarial Activity of Croton macrostachyus Stem Bark Extracts against Plasmodium berghei In Vivo Resveratrol Induces Apoptosis-Like Death and Prevents In vitro and In vivo Virulence of Entamoeba histolytica Phenotypic and Transcriptional Profiling in Entamoeba histolytica Reveal Costs to Fitness and Adaptive Responses Associated With Metronidazole Resistance Atg8 Is Involved in Endosomal and Phagosomal Acidification in the Parasitic Protist Entamoeba histolytica Entamoeba histolytica: Apoptosis Induced In vitro by Nitric Oxide Species Differentiation of Entamoeba histolytica: A Possible Role for Enolase Cysteine Proteases in Protozoan Parasites Entamoeba histolytica: Response of the Parasite to Metronidazole Challenge on the Levels of mRNA and Protein Expression Effect of the Sesquiterpene Lactone Incomptine A in the Energy Metabolism of Entamoeba histolytica Programmed Cell Death in Entamoeba histolytica Induced by the Aminoglycoside G418 Chemical Composition and Amoebicidal Activity of Croton Pallidulus, Croton Ericoides, and Croton Isabelli (Euphorbiaceae) Essential Oils Differential Expression of Pathogenic Genes of Entamoeba histolytica vs E. dispar in a Model of Infection Using Human Liver Tissue Explants Chemical Constituents from Croton Species and Their Biological Activities Conflict of Interest: The authors declare that the research was conducted in the